Bi-Ethnic Male Population: The SAfrEIC Study
Ruan Kruger1*, Rudolph Schutte1, Hugo W. Huisman1, Peter Hindersson2, Michael H. Olsen1,3, Jesper Eugen-Olsen4, Aletta E. Schutte1
1 Hypertension in Africa Research Team (HART); Department of Physiology, North-West University, Potchefstroom, North-West Province, South Africa, 2 Department of Biochemistry, Hospital Vendsyssel, Hjørring, Denmark,3 Cardiovascular Prevention Clinic, Department of Endocrinology, Odense University Hospital, University of Southern Denmark, Odense, Denmark,4 Clinical Research Centre 136, Copenhagen University, Hvidovre Hospital, Hvidovre, Denmark
Abstract
Objective and design:This cross-sectional study aimed to investigate associations between a marker of cardiac strain, the N-terminal prohormone B-type natriuretic peptide (NT-proBNP), and inflammation as reflected by either a conventional or novel inflammatory marker in a bi-ethnic South African cohort.
Methods and subjects: We measured NT-proBNP, C-reactive protein (CRP) and plasma-soluble urokinase plasminogen activator receptor (suPAR) levels along with conventional biomarkers in black (n = 117) and white (n = 116) men.
Results: NT-proBNP, CRP and suPAR levels were higher in black compared to white men. NT-proBNP was significantly associated with both CRP (r = 0.38; p = 0.001) and suPAR (r = 0.42; p,0.001) in black men only. After full adjustment in multiple regression analyses, the above associations of NT-proBNP with CRP (b = 0.199; p = 0.018) and suPAR (b = 0.257; p,0.01) were confirmed in black men.
Conclusion:These results suggest that a low-grade inflammatory state as reflected by both a conventional and novel marker of inflammation may contribute to higher cardiovascular risk as reflected by the associations obtained with a marker of cardiac strain in black South African men.
Citation: Kruger R, Schutte R, Huisman HW, Hindersson P, Olsen MH, et al. (2013) NT-proBNP, C-Reactive Protein and Soluble uPAR in a Bi-Ethnic Male Population: The SAfrEIC Study. PLoS ONE 8(3): e58506. doi:10.1371/journal.pone.0058506
Editor: Vladimir N. Uversky, University of South Florida, United States of America Received December 14, 2012; Accepted February 5, 2013; Published March 13, 2013
Copyright: ß 2013 Kruger et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: The SAfrEIC study was supported by the South African National Research Foundation Grant (GUN 2073040), the Medical Research Council (South Africa) and the Africa Unit for Trans-disciplinary Health Research of the North-West University (Potchefstroom campus, South Africa). The funding parties had no role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing Interests: The authors have declared that no competing interests exist. * E-mail: ruan.kruger@nwu.ac.za
Introduction
High morbidity and mortality among the black population in South Africa is a major concern due to the high prevalence of communicable and non-communicable diseases, especially in communities of low socio-economic standing with limited healthcare facilities [1]. A low-grade inflammatory state, height-ened by lifestyle and environmental factors, is believed to underlie the elevating adverse health outcomes observed in black patients [2]. The biological effects of pro-inflammatory cytokines and other components of inflammation are augmented by acute or chronic cardiovascular insults [3]. Pro-inflammatory cytokines, acute-phase reactants as well as cell adhesion and signaling molecules such as plasma-soluble urokinase plasminogen activator receptor (suPAR) and C-reactive protein (CRP) seem to play a role in mediating low-grade inflammation [3].
CRP, which reflects systemic inflammation, is elevated in acute heart failure and N-terminal prohormone B-type natriuretic peptide (NT-proBNP), reflecting cardiac strain, are proposed reliable risk markers of cardiovascular disease as well as good predictors of cardiovascular morbidity and mortality [4], [5], [6]. In addition, a novel marker of inflammation and subclinical
atherosclerosis (suPAR) is associated with the risk of developing cardiovascular disease [7], and is also suggested to be an independent marker of subclinical organ damage and increased cardiovascular risk [8].
The associations of NT-proBNP with markers of inflammation have been studied in part in white populations of American and European descent [7], [9], [10], [11], but little is known about these associations in black populations. The aim of this study was therefore to investigate whether subclinical cardiovascular damage assessed by NT-proBNP is associated with low-grade inflammation as reflected by a conventional and novel inflammatory marker.
Methods Study population
Ethics Statement. The SAfrEIC study was approved (06M01) by the Ethics Review Board of the North-West University and the study protocol conformed to the ethical guidelines of the Declaration of Helsinki (2008) for investigation of human participants. This cross-sectional study formed part of a larger South African investigation on the role of Sex, Age and Ethnicity on Insulin sensitivity and Cardiovascular function (SAfrEIC) study
that involved 382 black and 372 white participants from the North West province of Southern Africa. This sub-study included 117 black and 116 white men after excluding all patients who were using antihypertensive or anti-inflammatory medication (n = 41) and those infected with HIV (n = 55).
Clinical procedures
Approximately 10 to 20 recruited participants visited the Metabolic Unit facility daily at the Potchefstroom campus of the North-West University over a period of seven weeks. Each participant gave written informed consent to take part in the study after all the procedures were comprehensively explained. A participant sheet guided the participants through the different research stations where various measurements were performed. Basic health and demographic questionnaires were completed during the morning. An informative description regarding the results of the health assessment was given to each participant at the end of the study. In the event where abnormalities became evident (e.g. hypertension or diabetes), the participant was advised to visit their local clinic, hospital or physician.
Cardiovascular measurements
Duplicate office blood pressure measurements were taken with the Omron HEM-757 (Omron, Kyoto, Japan) apparatus. The first blood pressure measurement was taken after an initial 10 minute resting period and a second measurement was taken 5 minutes after the first. Pulse pressure was subsequently calculated. Participants with a systolic (SBP) $140 mmHg and/or diastolic blood pressure (DBP) $90 mmHg were considered hypertensive [12]. Heart rate and Windkessel arterial compliance were determined with the Finometer apparatus (FMS, Finapres Measurement Systems, Amsterdam, the Netherlands) [13], [14]. The pulse wave velocity (PWV), as arterial stiffness marker, was measured with the Complior SP Acquisition system (Artech-Medical, Pantin, France).
Anthropometric measurements
Body height was measured to the nearest 1.0 cm by using the Invicta Stadiometer (Invicta Plastics 1465, London, UK) and body weight to the nearest 0.1 kg (Precision Health Scale, A & D Company, Japan). Subsequently, the body mass index (BMI) was calculated for each participant. The waist circumference was measured at the midpoint between the lowest rib and the top of the iliac crest with a Holtain non-stretchable, flexible metal measuring tape [15].
Biochemical measurements
Participants were requested to fast for a minimum of eight hours. Fasting lipids (total cholesterol (TC), high-density lipopro-tein cholesterol (HDL), and triglycerides (TG)), serum glucose, c-glutamyl transferase, creatinine and high-sensitivity serum CRP were determined with the Konelab autoanalyzer (Thermo Fisher Scientific, Vantaa, Finland). Low density lipoprotein cholesterol (LDL) was determined with the Friedewald formula: LDL = TC – HDL – TG/2.17. Insulin was determined with the ST AIA-PACK IRI kit (TOSOH AIA, Inc., Toyama, Japan; catalogue no. 025260) using a two-site immuno-enzymometric assay. Serum cotinine was determined with the IMMULITE 2000 nicotine metabolite assay (Siemens Medical Solutions Diagnostics, Los Angeles, CA). The Elecsys proBNP sandwich immunoassay was used on an Elecsys 2010 (Roche Diagnostics, Mannheim, Germany) to determine the serum NT-proBNP concentration of each participant. Plasma (EDTA) suPAR levels were measured
using the suPARnosticH ELISA kit (ViroGates, Copenhagen, Denmark). Human immunodeficiency virus status was determined directly after blood sampling with rapid tests according to the protocol of the National Department of Health of South Africa. Serum was used for testing with the First Response Test (PMC Medical, India) and was repeated with the Pareeshak test (BHAT Bio-tech India) to confirm the results.
Statistical analyses
Statistica software v10.0 (StatSoft, Inc., Tulsa, OK, USA) was used for database management and statistical analyses. The normal distribution of the variables was tested prior to any further statistical analyses. Variables that deviated from normality (NT-proBNP, CRP, suPAR, c-glutamyl transferase, blood glucose and cotinine) were logarithmically transformed. Associations of NT-proBNP with markers of inflammation were tested for interaction with ethnicity by performing the appropriate interaction terms. Chi-square tests (x2) were used to compare proportions and
independent t-tests to compare the means of continuous variables. We plotted unadjusted associations between NT-proBNP and markers of inflammation in single regression analysis. We divided CRP and suPAR values into quartiles to explore associations with NT-proBNP levels, while adjusting for SBP and arterial compli-ance in analysis of covaricompli-ance (ANCOVA). A standard multiple regression analyses were performed to investigate independent associations between NT-proBNP and inflammatory markers. Several covariates were considered for entry into the regression model including age, BMI, SBP, arterial compliance, serum creatinine, c-glutamyl transferase, fasting glucose, total cholesterol to high density lipoprotein cholesterol ratio and cotinine. Probability values of a#0.05 were considered statistically signif-icant.
Results
Detailed clinical and basic population characteristics are presented in Table 1. The total population was stratified by ethnicity, due to significant interactions on the main effects of ethnicity on the associations of NT-proBNP with CRP (F(233) = 27.02; p,0.0001) and suPAR (F(233) = 30.3; p,0.0001). The black men were older (p = 0.003) and smoked more compared to the white men (p,0.0001). This was also supported by the higher cotinine levels (p,0.0001). The self-reported use of alcohol (82.2% vs. 76.3%; p = 0.26) was similar, but the levels of c-glutamyl transferase was higher in the black men (p,0.0001). Metabolic risk factors including BMI, serum glucose and lipid levels were lower in the black men. Mean levels of NT-proBNP (p,0.0001), CRP (p = 0.038) and suPAR (p,0.0001) were higher in the black compared to white men.
In single regression analysis (Figure 1), NT-proBNP correlated positively with both CRP (r = 0.38; p,0.001) and suPAR (r = 0.42; p,0.001) in black men only. By plotting NT-proBNP by quartiles of CRP and suPAR in both black and white men (Figure 2), with adjustments for SBP and arterial compliance, the relationships above were supported further in the black men (CRP; p for trend = 0.018 and suPAR; p for trend = 0.002). Again, no associations were observed in the white men (CRP; p for trend = 0.14 and suPAR; p for trend = 0.74).
The independent associations between NT-proBNP and inflammatory markers are shown in Table 2. After adjusting for age, BMI, SBP, arterial compliance, serum creatinine and c-glutamyl transferase (variables that entered the model), the positive associations with CRP (p = 0.018) and suPAR (p = 0.007) were
confirmed and remained non-significant in the white men (CRP; b = 20.017, p = 0.86 and suPAR; b = 0.121, p = 0.23).
CRP and suPAR levels were also compared after adjusting for BMI, since the BMI differed largely between these groups. After this adjustment, the initial difference between black and white men remained for both CRP (2.32 mg/l vs. 0.73 mg/l; p,0.001), and suPAR (2.97 ng/ml vs. 1.99 ng/ml; p,0.001). It is also notewor-thy to mention that the mean blood pressures of the black men were high normal compared to white men with optimal pressures. By performing ANCOVA with adjustments for BMI, SBP, cotinine and c-glutamyl transferase the initial difference in CRP levels between black and white men disappeared (1.68 mg/l vs. 1.01 mg/l; p = 0.17). None of these variables seem to alter the difference in mean suPAR levels in black or white men (2.67 ng/ ml vs. 2.20 ng/ml; p,0.01).
Discussion
This study investigated the associations of NT-proBNP with CRP and suPAR in black and white South African men.
NT-proBNP associated positively with both inflammatory markers in black men. However, this relationship was absent in the white group. It is known that CRP reflects metabolic inflammation with its relation to BMI and lipids [16], while suPAR may be more related to cell-specific immune activation of the circulation [17]. Our results confirm the conclusion of a previous study by Jensen et al. that suggested a positive relationship between NT-proBNP and inflammatory markers including CRP, orosomucoid, haptoglobu-lin and alpha1-antitrypsin in European (Swedish) men and woman [11]. No study investigated the relationship between NT-proBNP and suPAR; however Eugen-Olsen et al. investigated the potential of suPAR as a marker of adverse cardiovascular outcome in over 2500 Danish men and women. From those results, suPAR associated with an increased risk of cardiovascular disease, cancer, type 2 diabetes and mortality, more strongly in men than in women [7]. Our study is the first to investigate NT-proBNP, CRP and suPAR in a bi-ethnic cohort from South Africa. Therefore, our results suggest that a potential low-grade inflammatory state in black men may predispose them to premature development of subclinical cardiac strain and future cardiovascular events.
Increased levels of the cardiac hemodynamic volume load biomarker, NT-proBNP, reflect the risk of developing left ventricular dysfunction and congestive heart failure [18]. In addition, elevated CRP and suPAR levels indicate active systemic as well as low-grade inflammation, especially in atherosclerotic progression [19], [20]. Therefore, the associations of NT-proBNP with both these markers in black men suggest the link between the potential developments of subclinical cardiac damage in unison with early onset atherosclerosis. This relationship might also explain the higher systolic pressure and lower arterial compliance initially seen. Elevated concentrations of inflammatory markers are generally the result of infection, whether it is a simple acute cold or flu or because of more severe chronic conditions such as tuberculosis and HIV [21], [22]. In this study population, the levels of both NT-proBNP and inflammatory markers were not abnormally elevated. Yet the associations obtained in this study suggest that even low concentrations of inflammatory markers may contribute to elevated risk of cardiovascular damage and possible future cardiac events in the black male group. Conversely, white men exhibited higher levels of lipids and had higher mean BMI, but the lack of association between NT-proBNP and inflammatory markers, might suggest that some intrinsic cardioprotective mechanism(s) may be at work or early onset alterations are not prevalent and warrant further investigation.
The underlying and combined mechanisms relating NT-proBNP to CRP and suPAR in cardiovascular disease are not well understood and we can therefore only speculate to explain our findings. A cascade of contributing factors is involved in the poor cardiovascular state of the black South African population. Among these factors are adverse lifestyle choices which include alcohol misuse, insufficient dietary intake and excessive smoking. In turn, these factors contribute to alterations in hemodynamic and metabolic processes after which systemic inflammation becomes unavoidable [23], [24], [25]. This is in line with the known risk of cardiovascular disease among black South Africans [26]. With the development of systolic and diastolic dysfunction, due to obesity, lifestyle or predisposition, the volume load of the ventricles increases. This elevation in volume load results in cardiac myocyte stretch and stimulates the release of NT-proBNP [27], [28], [29]. Normally, the natriuretic peptide clearance receptor type C and the kidneys maintain the concentrations of BNP and its amino fragment to restore the equilibrium of the natriuretic peptide system and its effects [30]. However, once the heart is subjected to chronic myocyte stretch because of multiple components escalat-Table 1. Clinical and basic population characteristics of the
bi-ethnic male cohort.
African Caucasians p–value n = 117 n = 116
Age, years 41.4613.8 36.3611.7 0.003 Body mass index, kg/m2
20.464.2 27.865.0 ,0.0001 Biochemical analyses
NT-proBNP, ng/ml 29.6 (5.5–187.8) 10.9 (5.1–44.7) ,0.0001 C-reactive protein, mg/l 1.73 (0.007–22.86) 1.02 (0.007–9.22) 0.038 Soluble uPAR, ng/ml 2.95 (1.66–5.00) 2.02 (1.32–3.21) ,0.0001 Serum creatinine,mmol/l 63.9610.2 71.4610.5 ,0.0001 Serum glucose, mmol/l 4.97 (4.03–6.42) 5.54 (4.59–7.13) ,0.0001 TC:HDL, mmol/l 2.8861.08 5.2462.07 ,0.0001 Triglycerides, mmol/l 1.0760.55 1.5860.97 ,0.0001 LDL, mmol/l 2.2260.89 3.8661.37 ,0.0001 Insulin,mU/ml 4.9465.17 10.169.1 ,0.0001 Cardiovascular measurements Systolic blood pressure, mmHg
130.4620.6 121.7611.0 ,0.0001 Diastolic blood pressure,
mmHg 84.4613.7 77.668.1 ,0.0001 Pulse pressure, mmHg 46.1611.5 44.168.5 0.13 Heart rate, bpm 67.9614.5 66.169.1 0.25 Arterial compliance, ml/ mmHg 1.6760.51 2.5360.50 ,0.0001 Hypertension status, n (%) 44 (37.6) 8 (6.8) ,0.0001 Lifestyle Smoking, n (%) 87 (74.4) 25 (21.2) ,0.0001 Cotinine, ng/ml 115.9 (9.0–500.0) 18.3 (9.0–371.0) ,0.0001 Alcohol use, n (%) 97 (82.2) 90 (76.3) 0.26 c-Glutamyl transferase, U/l 79.5 (20.7–487.2) 35.5 (17.7–101.2) ,0.0001 Values are arithmetic mean 6 SD, geometric mean (5th
and 95th
percentiles) or number of participants. Abbreviations: TC:HDL – total cholesterol to high density lipoprotein cholesterol ratio; uPAR – urokinase plasminogen activator receptor.
ing in volume overload and augmented NT-proBNP concentra-tions, CRP and suPAR release are augmented by the expression of interleukin-6. The urokinase plasminogen activator will bind to its receptor (uPAR) to convert plasminogen into active plasmin [31]. Plasmin, in turn, has a direct effect on extracellular matrix degradation and can also convert pro-matrix metalloproteinases into active matrix metalloproteinases [32]. Metalloproteinases contribute to extracellular matrix degradation and ultimately to invasion of pro-inflammatory components [31]. As a result of either a systemic inflammatory or acute phase response, or also extracellular matrix remodelling, the heart is subjected to ventricular hypertrophy due to increased volume overload [33].
Our study has certain limitations. It was cross-sectional and therefore causality cannot be inferred due to confounding variables or unknown factors that were associated with both NT-proBNP and inflammation. The black men in this study were from a low socio-economic class (although all participant were
from the same geographical region), which could have rendered these subjects as high risk for developing disease, due to limited healthcare provision. However, no interactions were observed with socio-economic standing. NT-proBNP is known as a stable and sensitive marker of cardiac function, including right ventricular dysfunction [34], left ventricular systolic dysfunction, and early cardiac alterations [35]. NT-proBNP was therefore used only as a marker of potential cardiac damage. Echocardiography data was not available for this study. However, this was a well-designed study supervised under controlled conditions, and contributes to the limited literature available on NT-proBNP and its associations with inflammatory markers in a South African population. Furthermore, this result is clinically relevant and suggests that if intervention does not substantiate the risk observed in this black population, in due time they may be more prone to develop early subclinical cardiovascular damage and potential detrimental cardiac events.
Figure 1. Single regression analyses of NT-proBNP with markers of inflammation in black and white men. doi:10.1371/journal.pone.0058506.g001
Figure 2. NT-proBNP levels by quartiles of CRP and suPAR, adjusted for systolic blood pressure and arterial compliance. Probability denoted significance for trend; {p,0.01 (Q1vs. Q4).
In conclusion, NT-proBNP persistently associated with CRP and suPAR in black men, but not in white men. Our result suggests that a low-grade inflammatory state may potentiate adverse changes in hemodynamic strain on the heart. This is in line with the higher prevalence of hypertension and early onset hemodynamic alterations known to this group of black men. However, these findings need confirmation in larger prospective and experimental studies to identify potential mechanisms of early onset cardiovascular changes.
Acknowledgments
We sincerely thank Roche Diagnostics for supplying the NT-proBNP kits, as well as all the participants in this study, the Hypertension in Africa Research Team staff and postgraduate students that contributed to this study.
Author Contributions
Conceived and designed the experiments: RK RS HWH AES. Performed the experiments: RK PH MHO JE RS HWH AES. Analyzed the data: RK RS AES HWH MHO. Contributed reagents/materials/analysis tools: PH MHO JE RS HWH AES. Wrote the paper: RK RS MHO HWH AES JE PH.
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Table 2. Multiple regression analysis of NT-proBNP with CRP and suPAR in African men.
CRP, mg/l suPAR, ng/ml R2 0.43 0.44 Adjusted R2 0.39 0.41 Standard b (95% CI) NT-proBNP, ng/ml 0.199 (0.042 to 0.356)* 0.257 (0.088 to 0.425){ Age, years 0.559 (0.279 to 0.839){ 0.515 (0.242 to 0.788){
Body mass index, kg/m2
20.123 (20.298 to 0.053) 20.142 (20.311 to 0.026) Systolic blood pressure, mmHg 0.393 (0.188 to 0.497){
0.393 (0.193 to 0.592){
Arterial compliance, ml/mmHg 0.276 (20.057 to 0.608) 0.222 (20.101 to 0.545) Serum creatinine,mmol/l 20.191 (20.349 to 20.033)* 20.145 (20.305 to 0.015) c-Glutamyl transferase, U/l 20.096 (20.264 to 0.072) 20.185 (20.357 to 20.013)* Superscript symbol denotes significance for:
*p#0.05;
{
p#0.01;
{
p#0.001.
Abbreviations: CI – confidence intervals; TC:HDL – total cholesterol to high density lipoprotein cholesterol ratio. doi:10.1371/journal.pone.0058506.t002
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